首页> 外文期刊>The Journal of molecular diagnostics: JMD >Triplet repeat primed PCR simplifies testing for huntington disease
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Triplet repeat primed PCR simplifies testing for huntington disease

机译:三重重复引物PCR简化了亨廷顿病的检测

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Diagnostic and predictive testing for Huntington disease (HD) requires an accurate determination of the number of CAG repeats in the Huntingtin (HHT) gene. Currently, when a sample appears to be homozygous for a normal allele, additional testing is required to confirm amplification from both alleles. If the sample still appears homozygous, Southern blot analysis is performed to rule out an undetected expanded HTT allele. Southern blot analysis is expensive, time-consuming, and labor intensive and requires high concentrations of DNA. We have developed a chimeric PCR process to help streamline workflow; true homozygous alleles are easily distinguished by this simplified method, and only very large expanded alleles still require Southern blot analysis. Two hundred forty-six HD samples, previously run with a different fragment analysis method, were analyzed with our new method. All samples were correctly genotyped, resulting in 100% concordance between the methods. The chimeric PCR assay was able to identify expanded alleles up to >150 CAG repeats. This method offers a simple strategy to differentiate normal from expanded CAG alleles, thereby reducing the number of samples reflexed to Southern blot analysis. It also provides assurance that expanded alleles are not routinely missed because of allele dropout.
机译:亨廷顿病(HD)的诊断和预测测试要求准确确定亨廷顿(HHT)基因中CAG重复的数量。当前,当样品看起来对正常等位基因是纯合子时,需要额外的测试以确认来自两个等位基因的扩增。如果样品仍显示为纯合子,则进行Southern印迹分析以排除未检测到的扩展HTT等位基因。 Southern印迹分析昂贵,费时且费力,并且需要高浓度的DNA。我们开发了一种嵌合PCR流程,以帮助简化工作流程;真正的纯合等位基因可通过此简化方法轻松区分,并且只有非常大的扩展等位基因仍需要进行Southern印迹分析。使用我们的新方法分析了先前使用不同片段分析方法运行的246个HD样本。所有样品均已正确进行基因分型,从而使方法之间的一致性达到100%。嵌合PCR测定法能够鉴定高达> 150个CAG重复序列的扩展等位基因。该方法提供了一种简单的策略,可以区分正常的和扩展的CAG等位基因,从而减少了反映到Southern印迹分析的样品数量。它还可以确保不会因缺失等位基因而经常错过扩增的等位基因。

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